Histone-lysine acetylation is a vital chromatin post-translational modification involved in the epigenetic regulation of gene transcription. Bromodomains bind acetylated lysines, acting as readers of the histone-acetylation code. Competitive inhibitors of this interaction have antiproliferative and anti-inflammatory properties. With 57 distinct bromodomains known, the discovery of subtype-selective inhibitors of the histone-bromodomain interaction is of great importance. We have identified the 3,5-dimethylisoxazole moiety as a novel acetyl-lysine bioisostere, which displaces acetylated histone-mimicking peptides from bromodomains. Using X-ray crystallographic analysis, we have determined the interactions responsible for the activity and selectivity of 4-substituted 3,5-dimethylisoxazoles against a selection of phylogenetically diverse bromodomains. By exploiting these interactions, we have developed compound 4d, which has IC(50) values of
CREB-Binding Protein
,Cell Cycle Proteins
,Crystallography, X-Ray
,Cytotoxins
,HeLa Cells
,Histones
,Humans
,Isoxazoles
,Ligands
,Lysine
,Models, Molecular
,Molecular Mimicry
,Molecular Structure
,Nuclear Proteins
,Phenylethyl Alcohol
,Protein Binding
,Protein Serine-Threonine Kinases
,Protein Structure, Tertiary
,Stereoisomerism
,Structure-Activity Relationship
,Transcription Factors
